Rhizobacterial Colonization and Management of Bacterial Speck Pathogen in Tomato by Pseudomonas spp.

Plants and soil microorganisms interact at every stage of growth. Pseudomonas spp. are highly regarded for their ability to increase crop production and protection from diseases. The aim of this study is to understand the mechanisms of the rhizobacterial colonization of tomato roots via chemotaxis assay and the activation of tomato resistance against the pathogenic bacterium, Pseudomonas syringae pv. tomato DC3000 (Pst). The capillary assay was used to evaluate the chemotaxis response of PGPRs (plant growth-promoting rhizobacteria). The activities of defense enzymes and the expressions of PR (pathogenesis-related) genes were measured using real-time qPCR. Chemotactic responses to malic and citric acids (the most important root exudates found in different plant species) at low concentrations varied substantially among the rhizobacterial isolates (63 species). Beneficial isolates including Pseudomonas resinovorans A5, P. vranovensis A30, P. resinovorans A28, P. umsongensis O26, P. stutzeri N42, and P. putida T15 reacted well to different concentrations of root exudates. P. putida T15 demonstrated the most potent anti-Pst activity. At three and six days after inoculation, the greatest levels of polyphenol oxidase and peroxidase activity were reported in the A5 and T15 groups. In tomato, transcript levels of four PR (pathogenesis-related) genes were elevated by rhizobacterial treatments. PGPR isolates alone or in combination with BABA (β-amino butyric acid) up-regulated the transcriptions of PR1, PR2, LOX, and PAL genes. Treatments with N42 and T15 resulted in the greatest improvements in tomato growth and yield traits. In conclusion, the results explain the mechanisms of rhizobacterial colonization for the improved management of Pst. Rhizobacterial isolates play a role in tomato’s resistance to Pst via salicylic acid and jasmonic acid pathways.


Introduction
Rhizobacteria that enhance plant development and health are called PGPR (plant growth-promoting rhizobacteria) [1,2]. Biocontrol agents, especially PGPR, may act against different pathogens. The activation of plant growth by PGPR occurs through changing plant hormone concentrations, nutrient facilitation by biological N 2 fixation, inorganic phosphate solubilization, organic phosphate mineralization, and siderophores formation [3][4][5][6]. Antibiosis against phytopathogens, systemic resistance stimulation in plants, and the regulation of the growth of phytopathogens by forming iron-limiting conditions via the production of siderophores are examples of indirect mechanisms that reduce the effect of phytopathogens on plant growth [7]. PGPR have been utilized in commercial applications for disease biocontrol and phytoremediation, such as Pseudomonas putida [8]. Biofertilizers, evaluate the effect of the most effective PGPR strains in terms of chemotactic activity on tomato growth and resistance against Pst, and to explore the various mechanisms involved in the resistance induction against Pst using real-time quantitative PCR analysis.

Materials and Methods
2.1. Chemotaxis Activity of PGPRs 2.1.1. Collecting Root Exudates RE were collected [33]. Tomato seeds (Lycopersicon esculentum cv. Pantelosa), obtained from the Ministry of Agriculture, Egypt, were sterilized using NaOCl (sodium hypochlorite solution at 2% v/v, for 2 min) followed by washing three times in SDW (sterile distilled water). In a Petri dish, seeds (100 seeds) were put on Hoagland solution-wetted filter papers in the darkness at 25 • C for germination. Exudates from the roots were gathered in a magnate stirrer with a perforated tray filled with 80 mL of Hoagland solution. Eighty germinated seedlings with their roots in the solution were put on the tray. Exudates were obtained by filtration through Whatman No. 3 filter papers after 1 week of growth at 18 • C to eliminate solid plant contents, and then frozen quickly with liquid nitrogen. On solidified King's B medium, a sample of exudates was taken directly from the magnate vessels and checked for contamination. The solid material was re-dissolved in 2 mL sterile water after the exudates were lyophilized. These exudates were purified through a 0.45 µm Millipore membrane to eliminate undissolved particles and deposited at −20 • C until needed. Samples were identified and confirmed using liquid chromatography-mass spectrometry (Agilent, Santa Clara, CA, USA) [34].

Chemotactic Response of Bacterial Isolates to Organic Acids in a "Drop" Assay
The "drop" assay was utilized to conduct chemotaxis experiments with slight modifications [35]. After 24 h of incubation on Kings B medium, cells were diluted to 10 −2 in 150 mL of chemotaxis buffer containing 1% succinic acid. Forty ml of samples were resuspended in 12 mL chemotaxis buffer (100 mM potassium phosphate [pH7.0]/20 mM EDTA) when cells reached the early logarithmic phase (OD 600 of 0.12). To achieve a viscosity of 4000 cP in a 2% aqueous solution, the cell suspension was treated with an aqueous solution (up to 15 mL) of 1% hydroxypropyl methyl cellulose (Sigma-Aldrich). The resultant cell suspension was moved to a Petri dish (60 mm in diameter), where it produced a 3 mm thick layer. A drop (10 µL) of concentrated (50-fold) root exudates (citric acid (100 mM) and malic acid (100 mM) was placed into the dish's center at a concentration equal to or less than 0.1 M. After incubation at room temperature for 0.5 to 2 h, the plates were examined for the presence of a clear zone around the bacteria as criteria for a chemotactic reaction. Any turbidity rings that formed in the following 30 min were noted to determine the extent of the chemotactic reaction.

Chemotaxis Assay (Capillary Assay)
A modified capillary test based on Adler's method was used for the quantitative assessment of isolates' chemotaxis response to citric acid [36]. Sixty-three PGPR isolates were tested in this experiment. The identification of all strains was established by comparing 16S rDNA sequences to those of the strains. The pathogen P. syringae pv. tomato DC3000 and rhizobacterial isolates were obtained from Gifu university, Japan. The KB medium was used to grow the strains until they reached the log phase (OD 600 = 0.12). The cells were centrifuged and cleaned twice using chemotaxis buffer before being resuspended in the same buffer. Six mL of the above-mentioned cell suspension were placed on a Petri dish (60 mm in diameter). Three concentrations (1, 10, and 50 µM) of organic acids (malic acid and citric acid) were put into standard 2 µL capillary tubes and then immersed in the cell suspension. Static incubation at room temperature for 30 min after removing the capillary's contents into a sterile Eppendorf tube was performed. The suspension was diluted and then plated on KB plates. In KB plates cultured for 24 h at 30 • C, the CFU was measured. Each treatment was carried out three times in total.

Induction Treatments with PGPRs
Tomato seeds were sterilized and put on wetted filter papers in Petri dishes under sterilized conditions for germination at 25 • C in the dark. The vermiculite was packed into sterilized polypropylene bags and autoclaved for 6 min at 121 • C (three times at 12 h intervals). Sterilized pots (25 cm in diam) with autoclaved potting medium were planted with tomato seeds and irrigated three times/week. Two weeks of growing in a growth chamber at 30 • C with a 16 h light/8 h dark photoperiod were used to transplant the germinated seeds. PGPR isolates, attracted to low concentrations of citric acid, were grown in KB medium and shaken at 160 rpm and 30 • C for 24 h. The cells were collected by centrifugation at 12,000 rpm for 10 min, then washed with SDW and resuspended in 10 MgCl 2 . The harvested bacterial suspensions were adjusted to 1 × 10 8 CFU. Soil was inoculated with different bacterial suspensions. An additional treatment (booster) was conducted 1 day before pathogen inoculation by soil drenching with β-amino butyric acid (BABA). A stock solution of BABA (Syngenta Research, Triangle Park, NC, USA) at 0.33 M was used. P. syringae pv. tomato DC3000 inoculation was done as described by Elsharkawy et al. [37]. Five days after Pst inoculation, the severity of the disease was measured by measuring the area of infected leaves on a scale from 0 (no symptoms) to 100 (severe necrotic symptoms). The number of Pst was determined on tomato leaves [37].

Assessment of Defense-Related Enzymes
Enzyme extracts were produced using the approved procedures by Elsharkawy et al. [38]. Tomato leaf samples were collected and pulverized in a mortar and pestle containing liquid nitrogen at three and six days post Pst inoculation (DPI). After grinding for 30 s, the powder was homogenized in a mortar and pestle with 3 mL of sodium phosphate buffer pH 6.8 (0.01 M). A refrigerated centrifuge was used to clarify the filtrates for 15 min at 6000 rpm after filtering the triturated tissues through cheesecloth. The clear supernatant was used to measure defense enzymes using a spectrophotometer (DR 5000 UV-VIS-Hyxo).
The activity of peroxidase (POX) in the obtained samples was determined using spectrophotometric analysis. Although there are many different types of POX enzymes, we chose guaiacol as a marker for general POX activity. Phosphate buffer (2.5 mL, pH7.0) and 0.2 mL enzyme extract were added to all test tubes (2 sets). Guaiacol solution (1%, 0.2 mL) was added and stirred in the experimental set. For 15-20 min, both sets were kept at room temperature. Subsequently, the contents of all the test tubes were then carefully mixed with 0.1 mL of 0.3% H 2 O 2 . Distilled water (0.2 mL), 0.1 mL of 0.3 % H 2 O 2 , and 2.5 mL of phosphate buffer (pH 7.0) were used to prepare the blank. A spectrophotometer was used to measure the absorbance at 470 nm. Each measurement was repeated three times.
The enzyme extract was utilized to measure polyphenol oxidase activity (PPO). Using phosphate buffer (pH 7.3), the final volume of the extract was increased to 25 mL, and the filtrate was centrifuged for 1 h at 15,000 rpm. The fraction precipitated between 45 and 95%, and saturation was obtained and re-dissolved in phosphate buffer after an ammonium sulphate fractionation. The mixture was then dialyzed in cellulose dialysis tubing at 4 • C. The activities of catecholase and cresolase were assessed spectrophotometrically [39]. To test the catecholase activity, a 30 mM 4-methyl catechol (4MC) substrate in a sodium acetate buffer (10 mM, pH 4.5) was used. Regarding crude enzyme extract (1 mL), the reaction was initiated by adding 1 mL of the substrate and 3 mL of phosphate buffer (pH 7.3) to the mixture. A spectrophotometer was used to measure the change in absorbance at 400 nm.

Molecular Investigation
The Total RNA Purification Kit (Thermo Scientific, Fermentas (Waltham, MA, USA), #K0731) was used to extract RNA from tomato leaves according to the manufacturer's procedure. The Reverse Transcription Kit (Thermo Scientific, Fermentas, #EP0451) was used for cDNA synthesis. Template RNA (5 µL) was put to a sterile, nuclease-free tube on ice, followed by 0.5 µL Oligo dT, and the volume was increased to 12.5 µL using DEPCtreated water. On the nuclease-free tube holding the component of the first step, 4 µL of 5× reaction buffer, 0.5 µL of RiboLock RNase Inhibitor, 2 µL of dNTP Mix, and 1 µL of RevertAid TM H Minus Reverse Transcriptase were added. The mixture was gently mixed before being incubated at 42 • C for 60 min. To ensure that the quantities of RNA and cDNA are pure enough for real-time PCR, the concentrations were quantified. The Q5000 (UV-Vis spectrophotometer Q5000/USA) was used to perform all required measurements and computations automatically. The expression of target genes mRNAs was measured using real-time PCR with SYBR Green. The cDNA was amplified using 2× Maxima SYBR Green/ROX qPCR Master Mix (Thermo Scientific, USA, #K0221) and gene specific primers according to the manufacturer's procedure. Table 1 lists the primers used in the amplification, including pathogenesis-related genes of PR1, PR2, lipoxygenase (LOX), and Phenylalanine ammonia lyase (PAL). Firstly, the polymerase chain reaction (PCR) mixture was denatured at 94 • C for 5 min, followed by 40 cycles of denaturation for 30 s at 94 • C, annealing for 30 s at 55 • C, and extension for 30 s at 72 • C. The housekeeping gene (Ubectin 13) serves as a normalizer for calculating relative gene expression or fold change in the target gene. The 2 −∆∆Ct method was employed to equalize the quantities cycle threshold (Ct) of the target gene with the quantities Ct of the housekeeping gene [40]. In both the target and reference genes, the control group served as a calibrator, while the other groups served as test groups. Table 1. Forward and reverse primers sequence for pathogenesis-related genes.

Gene
Forward Primer Reverse Primer Size Accession Number TCCATCTCGTGCTCCGTCT GAACCTTTCCAGTGTCATCAACC 144 X58253

Plant Growth under Field Experiments
On a loamy soil, 15 treatments were applied in plots of 15 plants for a total of 225 tomato plants on a raised bed at a spacing of 0.55 m. Treatments were P. umsongensis O26, P. vranovensis A30, P. resinovorans A5, P. resinovorans A28, P. resinovorans A33, P. resinovorans A47, P. brassicacearum N6, P. brassicacearum N32, P. putida T15, P. stutzeri N42, P. putida C21, P. aeruginosa B30, P. alcaligenes B5, P. alcaligenes B16, and control. Tomatoes were planted in rows of 120 × 40 cm, with a row length of 25 m. The experiments used a split-plot design with a randomized complete block and were repeated three times. The plants were irrigated using the drip method. The application of 14 PGPR isolates (1 × 10 8 CFU/cm 3 ) was performed as soil drench at 2 days before pathogen inoculation [2]. Plants in the control group were treated with sterile water. Cumulative yield (kg/plant), plant height (cm), fresh weight (g), dry weight (g), number of branches, chlorophyll contents, number of fruits per plant, average fruit weight (g), leaf area (cm 2 ), number of flowers per plant, vitamin C (mg/100 g), titratable acidity, and total soluble solids (TSS, %) were all used to evaluate the growth enhancement by bacterial treatments.

Statistical Analysis
Means were used to represent all data. Fisher's least significant difference (LSD) test was employed to evaluate statistical significance [38]. The experiments were performed three times. All analyses were performed with a significance level of p ≤ 0.05 using XLSTAT PRO (statistical analysis software, Addinsoft 2016.02.270444 version, Paris, France).

Chemotaxis Activity of PGPRs
The chemotactic response of 63 bacterial isolates to malic and citric acids was investigated to identify the reason for the biocontrol agents' preferred colonization pattern ( Table 2). Isolates including P. resinovorans A5, P. resinovorans A47, P. umsongensis O26, P. putida C21, and P. putida T15 reacted well to both concentrations of root exudates (Table 2). B5 and B16, on the other hand, may be attracted to malic acid, but not to citric acid (Table 2).  PGPRs, particularly P. umsongensis O26, P. vranovensis A30, P. resinovorans A5, P. resinovorans A28, P. stutzeri N42, and P. putida T15, responded clearly to chemotaxis buffer concentrated root exudates (malic acid and citric acid), in contrast to the non-treated control (Table 3). B11 and C37 induced an inconspicuous chemotactic response to citric acid. Neither B5 nor B16 elicited a reaction ( Figure 1). When examined in 10-µL drops at concentrations of 100 mM, the major amino acids found in tomato root exudate, L-glutamic acid, L-aspartic acid, L-leucine, L-isoleucine, and L-lysine, all elicited a response of PGPR isolates. The threshold concentration of organic acids that may cause chemotaxis was determined by testing various concentrations of organic acids in 10-µL drops. Citric acid and malic acid responses were started at doses as low as 10 to 50 mM ( Table 3). The best isolates in the responses to low doses of citric and malic acids were shown compared with the isolates Pseudomonas alcaligenes B5 and Pseudomonas alcaligenes B16 (Table 3).    The chemotactic response of PGPRs to different doses of malic and citric acids was determined using a modified quantitative capillary chemotaxis test. Citric acid, found in tomato root exudates, was shown to attract P. umsongensis O26, P. vranovensis A30, P. resinovorans A5, P. resinovorans A28, P. stutzeri N42, and P. putida T15 at concentrations ranging from 1 to 50 mM (Figure 2). Malic and citric acids (1, 10, and 50 mM) showed clear positive and concentration-dependent chemotactic behavior in PGPR strains, with the most effective concentration ranging from 10 to 50 mM ( Figure 2). Only B5 and B16 chemotactic responses were induced by malic acid at concentrations of 1, 10, and 50 mM, without any response toward all concentrations of citric acids (Figure 2). The chemotactic response of PGPRs to different doses of malic and citric acids was determined using a modified quantitative capillary chemotaxis test. Citric acid, found in tomato root exudates, was shown to a ract P. umsongensis O26, P. vranovensis A30, P. resinovorans A5, P. resinovorans A28, P. stu eri N42, and P. putida T15 at concentrations ranging from 1 to 50 mM ( Figure 2). Malic and citric acids (1, 10, and 50 mM) showed clear positive and concentration-dependent chemotactic behavior in PGPR strains, with the most effective concentration ranging from 10 to 50 mM ( Figure 2). Only B5 and B16 chemotactic responses were induced by malic acid at concentrations of 1, 10, and 50 mM, without any response toward all concentrations of citric acids (Figure 2).

Induction of Systemic Resistance against Pst by PGPR
Root treatment with PGPR resulted in induced systemic resistance (ISR) in tomato against Pst. The defensive mechanisms mediated by PGPR were described using a tomatobased model system. A screening procedure using root treatment was done to explore the

Induction of Systemic Resistance against Pst by PGPR
Root treatment with PGPR resulted in induced systemic resistance (ISR) in tomato against Pst. The defensive mechanisms mediated by PGPR were described using a tomatobased model system. A screening procedure using root treatment was done to explore the most effective PGPR strains in terms of chemotactic activity and, consequently, the most effective isolates against Pst. ISR against the pathogen was measured five days after a challenge by calculating disease severity as a percentage, and Pst proliferation was checked in the leaves. T15 had the most remarkable outcomes in terms of lowering disease severity (18.3%) and pathogen proliferation (14.5) (Figure 3). Among 14 PGPR isolates, the most efficient nine isolates were selected and used as dual treatments with BABA against Pst. Results showed that the treatments exhibited substantial suppression of disease symptoms without any symptoms of infection ( Figure 4). According to these findings, root dual treatments with BABA and P. umsongensis O26, P. resinovorans A5, P. resinovorans A33, P. resinovorans A47, P. brassicacearum N6, P. brassicacearum N32, and P. putida T15 were more resistant to Pst-caused foliar disease, and showed a considerable decrease in disease severity (7.

Effects of PGPR Treatments on Enzyme Activities in Plants Infected with Pst
Peroxidase and polyphenol oxidase activities at 3 and 6 days post-inoculation (DPI) in different PGPR treatments were presented in Table 4. PGPR isolates induced considerable increases in POX and PPO activity in tomato plants compared with the control treat- Among 14 PGPR isolates, the most efficient nine isolates were selected and used as dual treatments with BABA against Pst. Results showed that the treatments exhibited substantial suppression of disease symptoms without any symptoms of infection ( Figure 4). According to these findings, root dual treatments with BABA and P. umsongensis O26, P. resinovorans A5, P. resinovorans A33, P. resinovorans A47, P. brassicacearum N6, P. brassicacearum N32, and P. putida T15 were more resistant to Pst-caused foliar disease, and showed a considerable decrease in disease severity (7.8, 8.2, 8.4, 8.2, 8.3, 8.5, and 8.1%, respectively) and the proliferation of Pst in the leaves (5.1, 4.8, 5, 4.6, 4.6, 5, and 4.4, respectively) compared with control plants (52 and 45%, respectively). Among 14 PGPR isolates, the most efficient nine isolates were selected and used as dual treatments with BABA against Pst. Results showed that the treatments exhibited substantial suppression of disease symptoms without any symptoms of infection ( Figure 4). According to these findings, root dual treatments with BABA and P. umsongensis O26, P. resinovorans A5, P. resinovorans A33, P. resinovorans A47, P. brassicacearum N6, P. brassicacearum N32, and P. putida T15 were more resistant to Pst-caused foliar disease, and showed a considerable decrease in disease severity (7.8, 8.2, 8.4, 8.2, 8.3, 8.5, and 8.1%, respectively) and the proliferation of Pst in the leaves (5.1, 4.8, 5, 4.6, 4.6, 5, and 4.4, respectively) compared with control plants (52 and 45%, respectively).

Effects of PGPR Treatments on Enzyme Activities in Plants Infected with Pst
Peroxidase and polyphenol oxidase activities at 3 and 6 days post-inoculation (DPI) in different PGPR treatments were presented in Table 4. PGPR isolates induced considerable increases in POX and PPO activity in tomato plants compared with the control treat-

Effects of PGPR Treatments on Enzyme Activities in Plants Infected with Pst
Peroxidase and polyphenol oxidase activities at 3 and 6 days post-inoculation (DPI) in different PGPR treatments were presented in Table 4. PGPR isolates induced considerable increases in POX and PPO activity in tomato plants compared with the control treatment (Table 4). Additionally, it is clear from the data that POX and PPO activities were higher at 3 DPI than 6 DPI. PGPR isolates; P. resinovorans A5, P. resinovorans A33, P. resinovorans A47, P. stutzeri N42, P. putida T15, and P. putida C21 recorded the highest values of POX and PPO activities at 3 and 6 DPI (Table 4). PPO and POX activities were determined after 3 and 6 DPI in plants treated with both PGPR isolates and BABA or BABA alone ( Table 5). The obtained data showed that the most effective treatment was the dual treatment with T15 and BABA, which recorded 66.0 and 49.4 for POX at 3 and 6 DPI, and 45.4 and 41.1 for PPO at 3 and 6 DPI, respectively, and consequently caused higher reduction values of bacterial leaf speck disease than the untreated inoculated control (Table 5). Table 5. Activity of peroxidase and polyphenol oxidase enzymes (mg/mL −1 ) on tomato leaves that were treated by PGPRs and BABA.

Effects of PGPR Treatments on Plant Growth and Yield
The results revealed that bacterial treatments substantially impacted fruit production, vitamin C, and the number of fruits per plant (Tables 6 and 7). A significant increase in the yield was achieved using A5 (5.8 kg/plant), A30 (5.7 kg/plant), A47 (5.9 kg/plant), N6 (5.9 kg/plant), T15 (6.2 kg/plant) and C21 (5.9 kg/plant) as compared with the control (3.3 kg/plant) ( Table 6). PGPR-treated plants outperformed their untreated controls in terms of yield measures. Treatment with T15 exhibited the highest increase in the number of flowers and fruits and weight of fruits/plant compared with other isolates and control treatment. Additionally, the isolates P. resinovorans A5, P. resinovorans A47, P. brassicacearum N6, and P. putida C21 showed a higher number of fruits, and fruits weight/plant T15 had the most significant outcomes in terms of fresh and dry weights, plant height, number of branches, leaf area, and chlorophyll content, although there were substantial variations between treatments.  TSS, acidity, and vitamin C concentration were the fruit quality parameters examined. T15 treatment provided the highest vitamin C (137.3 mg/100 g) compared with the control treatment (120.2 mg/100 g). P. putida T15, P. stutzeri N42, P. vranovensis A30, P. resinovorans A5, and P. putida C21 had the same TSS levels (5.21, 5.19, 5.19, 5.22, and 5.18, respectively), with no statistically significant differences. All treatments were significantly higher than the control. Similar to vitamin C contents, A5, A30, A47, N6, N42, T15, and C21 treatments increased the acidity of tomato fruits (0.58, 0.57, 0.58, 0.58, 0.59, 0.58, and 0.57) compared to the control (0.47), respectively (Table 7).

Molecular Analysis of Defense Genes by Real-Time PCR
After treatment with PGPR isolates alone or in combination with BABA, real-time PCR was performed to assess the relative expression of four pathogenesis-related proteins encoded by the genes PR1 and PR2, LOX, and PAL. An evaluation of these genes' transcription levels in the treated tomato and the control was carried out. Nanodrop was used to evaluate the quality and concentration of total RNA, which revealed pure RNA with much higher quantities of RNA (ranging from 950 to 2050 ng/µL). The housekeeping gene encoding the elongation factor Ubectin 13 was utilized as an internal reference for normalization throughout the real-time PCR experiment, and data were represented as mean ± SEM.
Compared to control tomato plants, PGPR-treated tomato plants had a substantial increase in PR1 gene expression before Pst inoculation ( Figure 5). Plants treated with T15 + BABA showed the highest expression (34.06 folds). The amount of PR2 gene expression in PGPR-treated tomato plants was substantially higher than in control plants ( Figure 5). In addition, dual treatment with T15 and BABA resulted in the highest up-regulation of PR2 gene expression (31.56 folds), followed by dual treatments with N42 + BABA, A5 + BABA and O26 + BABA.

Discussion
We examined the chemo-a ractants in 63 root-colonizing rhizobacterial strains a The mean value of PR2 gene expression in PGPR-treated tomato plants was substantially higher than in the control plants ( Figure 5). Gene expression was not significantly different between O26 + BABA, A5 + BABA and A30 + BABA treatments. When comparing all treatments, dual treatment with T15 and BABA showed the highest expression of the PR1 gene than other treatments. PAL gene expression was significantly increased in plants treated with PGPR compared to the control ( Figure 5). T15 + BABA, N42 + BABA, and N6 + BABA were significantly more elevated than the other treatments in all groups. Furthermore, plants treated with T15 + BABA had a greater up-regulation of PAL gene expression than plants treated with N42 + BABA or N6 + BABA ( Figure 5).

Discussion
We examined the chemo-attractants in 63 root-colonizing rhizobacterial strains and evaluated their colonizing and chemotactic behavior. The movement of an organism in reaction to a chemical stimulation is known as chemotaxis. This is crucial because bacteria move toward the areas with the highest concentrations of food molecules (such as glucose). Carbon-based chemicals make up the majority of root exudates [41]. Soil microbes need organic acids which may serve as food and signal molecules [14]. The effects of malic and citric acids on the chemotactic response of PGPR were elucidated. The compositions of plant root exudates are closely linked to the chemotaxis response and colonization behavior of bacterial strains. This study offers valuable information with implications for co-evolution between plants and microorganisms in the same niche, as well as improved PGPR-strain selection for agricultural production applications. P. putida T15 has the genetic components (chemotaxis, adhesion structures, and antimicrobial activities) to colonize the rhizosphere effectively. Various concentrations of malic and citric acids were examined to establish the chemotaxis threshold concentration. Low quantities of malic and citric acids, such as 10 mM, elicited the response of PGPRs. Exudates stimulated chemotaxis, proliferation, and biofilm formation, which impacted B. amyloliquefaciens BNM339 colonization of soybean seeds [42]. The higher favorable reactivity of P. putida T15 to tomato root exudates may essentially explain its colonization behavior. Many different organic acids, such as citric and malic acids, are released simultaneously by the bacteria in the rhizosphere at the same time and have been associated with their function in phosphate solubilization.
Fourteen distinctly different PGPR isolates were utilized against Pst, and the protective effect and mechanism of the PGPR in tomato plants were elucidated. Our findings show that only PGPR treatment is sufficient to protect plants. In tomato, a mixture of PGPR and BABA substantially increased resistance to Pst. The number of symptomatic leaves, the proliferation of Pst in the leaves, and the severity of the disease were all decreased as a result of PGPR treatment. In tomato plants, the function of defensive signaling molecules has been investigated using real-time PCR. The fact that PGPR alone or in combination with BABA substantially upregulated the pathogenesis-related genes (PR1, PR2, LOX, and PAL) explains their importance in systemic resistance to Pst. ISR refers to the reduction in the severity or incidence of disease caused by PGPR-elicited host defenses that are spatially separated from pathogens [43]. The stimulation of PGPR in plants leads to indirect systemic resistance to pathogens [44,45]. In Arabidopsis and tobacco, the systemic resistance generated by the bacteria Serratia marcescens 90-166 or Pseudomonas fluorescens WCS417 is independent of SA accumulation [46]. P. aeruginosa 7NSK2, on the other hand, used the SA-dependent pathway to elicit ISR against Botrytis cinerea in tomato and Tobacco mosaic virus in tobacco [47]. Using Arabidopsis mutant lines, a model pathway for signal transduction in PGPR-mediated ISR was established [2]. ISR induced by PGPR is dependent on jasmonic acid (JA), ethylene, and SA, according to the proposed pathway [2]. The treatments P. putida T15 and P. putida T15 + BABA substantially reduced the severity of Pst (p ≤ 0.05). When compared to the control, PGPR isolates substantially enhanced all the tested plant growth parameters. Individual P. putida T15 treatment exhibited the most substantial increases in tomato growth and yield compared to other treatments. PGPR isolates outperformed the control in all plant growth and morphological parameters. PGPR has been shown to improve plant growth via a number of methods, including mineral phosphate solubilization, biological nitrogen fixation, plant hormone production, and stress reduction [5]. PGPR may also have an indirect impact on plant development by keeping pathogens from deleterious effects.
In conclusion, the processes by which the plant recognizes helpful microorganisms were addressed. Root exudates (malic and citric acids) attract beneficial rhizobacteria leading to the stimulation of defense response in tomato against Pst. These results are important for improving management strategies against plant pathogens.